Aldosterone induces clonal β-cell failure through glucocorticoid receptor
Fang Chen, Jia Liu, Yanyang Wang, Tijun Wu, Wei Shan, Yunxia Zhu and Xiao Han*
Key Laboratory of Human Functional Genomics of Jiangsu Province, Nanjing Medical University, 140 Hanzhong Road, Nanjing 210029, China.
*Corresponding author: Xiao Han, Ph.D. Mailing address: Key Laboratory of Human Functional Genomics of Jiangsu Province, NanjingMedicalUniversity, 140 Hanzhong Road, Nanjing, 210029, China.
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Reprints request should be addressed to Dr. Xiao Han.
Supplemental Figure-1. Aldosterone induced dysfunction and apoptosis of clonal-cell.Treatment withaldosterone (10, 100, 1000 nmol/l) for 24 h significantly decreased (A) insulin secretion (white bars,2 mmol/l glucose; black bars, 50 mmol/l KCl) and (B) insulin content of INS-1 cells. Similar effects on (C)insulin secretion (white bars,2 mmol/l glucose; gray bars, 20 mmol/l glucose; black bars, 50 mmol/l KCl) and (D) insulin content of rat islets wereobserved.Min6 cells (E) and INS-1 cells (F)were treated with different concentrations of aldosterone for 24 h, 48 h, and 72 h, and then MTT assays were performed. Aldosterone significantly inhibited viability of Min6 and INS-1 cells. (G) Treatment with aldosterone(10, 100, 1000 nmol/l) for 72 h significantly induced apoptosis of INS-1cells measured by staining with TUNEL and Hoechst. Apoptosis was determined by scoring the percentage of TUNEL-positive cells. About 2,000 cells were scored for each group in one experiment. *P < 0.05 and **P < 0.01, compared to control.
Supplemental Figure-2. Aldosterone induced impairement of INS-1 cells in a GR-dependent manner. After pretreatment with MR antagonist spironolactone (100 nmol/l) or GR antagonist RU486 (1 μmol/l) for 2 h, INS-1 cells were treated with the aldosterone for additional 24 h. The decrease of insulin secretion (A) and insulin content (B) in INS-1 cells induced by aldosterone were significantly reversed by RU486 pretreatment.(C) Transfected with 100 nmol/l GR siRNAs (001, 002, 003) in INS-1 cells for 24 h significantly downregulated GR protein expression. Similar results were obtained by transfected with MR siRNAs (001, 002, 003). After transfected with 100 nmol/l NC, si-GR (003) or si-MR (003) for 24 h, INS-1 cells were treated with aldosterone(100 nmol/l) for 24 h. The decrease of insulin secretion (D) and insulin content (E) in INS-1 cells induced by aldosterone were significantly reversed by transfected with si-GR. (F) Transfected with 100 nmol/l si-GR (003)significantly downregulated GR protein expressionin INS-1 cells for different time. (G) INS-1 cells were transfected with 100 nmol/l NC, si-GR (003) or si-MR (003) for 24 h, and then treated with aldosterone (100 nmol/l) for 72 h. The apoptosis of INS-1 cells induced by aldosterone were significantly reversed by transfected with si-GR. **P < 0.01, compared to control; ##P 0.01, compared toNC + aldosterone group.
Supplemental Figure-3.Up-regulation of MafA expression protects-cellsfrom aldosterone-induced impairment.(A)Min6 cells, INS-1 cells, mouse islets and rat islets were transfected with MafA over-expression plasmid (P-MafA) or MafA over-expression Adenovirus (Ad-MafA) for 24 h. Theoverexpression potencies of these plasmid and adenoviruses were confirmed by Western blotting.Transfection with P-MafAin INS-1 cells reversed the aldosterone-induced decrease of insulin secretion(B) and insulin content (C).Infection with Ad-MafAin rat islets reversed the aldosterone-induced decrease of insulin secretion (D) and insulin content(E). (F) Transfection with P-MafA reversed the aldosterone-induced apoptosis of INS-1 cells. **P < 0.01, compared to control. # P < 0.05 and ##P < 0.01, compared to C-plasmidor Ad-GFPcombined with aldosterone-treated group.
Supplemental Figure-4.The full western blot analysis of MafA expression in Min6, INS-1 and 293A cells was shown. After the treatment of aldosterone for 24h, the expression of MafA protein was determined in Min6, INS-1 and 293A cells. MafA was expressed in Min6 and INS-1 cells, but not 293A cells. Aldosterone treatment significantly inhibited MafA protein expression. Con: control, Ald: aldosterone.
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